4.6 Article

Myosin-X Induces Filopodia by Multiple Elongation Mechanism

Journal

JOURNAL OF BIOLOGICAL CHEMISTRY
Volume 285, Issue 25, Pages 19605-19614

Publisher

AMER SOC BIOCHEMISTRY MOLECULAR BIOLOGY INC
DOI: 10.1074/jbc.M109.093864

Keywords

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Funding

  1. NHLBI NIH HHS [R01 HL073050] Funding Source: Medline
  2. NIAMS NIH HHS [AR048898, R01 AR048526, R01 AR048898, AR048526] Funding Source: Medline
  3. NIDCD NIH HHS [DC006103, R01 DC006103] Funding Source: Medline

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Filopodia are actin-rich finger-like cytoplasmic projections extending from the leading edge of cells. Unconventional myosin- X is involved in the protrusion of filopodia. However, the underlying mechanism of myosin-X-induced filopodia formation is obscure. Here, we studied the movements of myosin-X during filopodia protrusion using a total internal reflection microscope to clarify the mechanism of myosin-X-induced filopodia formation. Myosin-X was recruited to the discrete site at the leading edge where it assembles with exponential kinetics before the filopodia extension. The myosin-X-induced filopodia showed repeated extension-retraction cycles with each extension of 2.4 mu m, which was critical to produce long filopodia. Myosin-X, lacking the FERM domain, could move to the tip as does the wild type. However, it was transported toward the cell body during filopodia retraction, did not undergo multiple extension-retraction cycles, and failed to produce long filopodia. During the filopodia protrusion, the single molecules of full-length myosin-X moved within filopodia. The majority of the fluorescence spots showed two-step photobleaching, suggesting that the moving myosin-X is a dimer. Deletion of the FERM domain did not change the movement at the single molecule level with the same velocity of similar to 600 nm/s as wild-type, suggesting that the myosin-X in filopodia moves without interaction with the attached membrane via the FERM domain. Based upon these results, we have proposed a model of myosin-X-induced filopodia protrusion.

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